BioMed Central Page 1 of 14 (page number not for citation purposes) Virology Journal Open Access Hypothesis Replicative Homeostasis: A fundamental mechanism mediating selective viral replication and escape mutation Richard Sallie* Address: Suite 35, 95 Monash Avenue, Nedlands, Western Australia, Australia Email: Richard Sallie* - sallier@mac.com * Corresponding author Abstract Hepatitis C (HCV), hepatitis B (HBV), the human immunodeficiency viruses (HIV), and other viruses that replicate via RNA intermediaries, cause an enormous burden of disease and premature death worldwide. These viruses circulate within infected hosts as vast populations of closely related, but genetically diverse, molecules known as "quasispecies". The mechanism(s) by which this extreme genetic and antigenic diversity is stably maintained are unclear, but are fundamental to understanding viral persistence and pathobiology. The persistence of HCV, an RNA virus, is especially problematic and HCV stability, maintained despite rapid genomic mutation, is highly paradoxical. This paper presents the hypothesis, and evidence, that viruses capable of persistent infection autoregulate replication and the likely mechanism mediating autoregulation – Replicative Homeostasis – is described. Replicative homeostasis causes formation of stable, but highly reactive, equilibria that drive quasispecies expansion and generates escape mutation. Replicative homeostasis explains both viral kinetics and the enigma of RNA quasispecies stability and provides a rational, mechanistic basis for all observed viral behaviours and host responses. More importantly, this paradigm has specific therapeutic implication and defines, precisely, new approaches to antiviral therapy. Replicative homeostasis may also modulate cellular gene expression. Background 1. Disease burden Hepatitis C (HCV), HBV and HIV are major causes of pre- mature death and morbidity globally. These infections are frequently life-long; Hepatitis viruses may result in pro- gressive injury to the liver and cirrhosis, and death from liver failure, or hepatocellular carcinoma, while HIV causes progressive immune depletion and death from the acquired immunodeficiency syndrome (AIDS). Together, these infections cause millions of premature deaths annu- ally, predominantly in "developing" countries. Other viruses replicating via RNA intermediaries cause similar morbidity among domestic and wild animal populations. While education, public health measures and vaccination (for HBV) have resulted in significant progress in disease control, therapy of established viral infection remains unsatisfactory. 2. Viral replication RNA viruses and retroviruses replicate, at least in part, by RNA polymerases (RNA pol ), enzymes that lack either fidel- ity or proofreading function [76]. During replication of hepatitis C HCV or HIV each new genome differs from the parental template by up to ten nucleotides [61] due to RNA pol infidelity that introduces errors at ~1 × 10 -5 muta- tions / base RNA synthesised. Published: 11 February 2005 Virology Journal 2005, 2:10 doi:10.1186/1743-422X-2-10 Received: 23 January 2005 Accepted: 11 February 2005 This article is available from: http://www.virologyj.com/content/2/1/10 © 2005 Sallie; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0 ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 2 of 14 (page number not for citation purposes) Viruses replicate by copying antigenomic intermediate templates and hence obey exponential growth kinetics, such that [RNA] t = [RNA] (t-1) e k , where [RNA] t is virus con- centration at time (t) and k a growth constant. However, because of RNA pol infidelity, wild-type (wt) virus will accumulate at [RNA wt ] t = [RNA wt ] (t-1) •(1-ρ)•K 1 and vari- ant forms (mt) at [RNA mt ] t ≈ ([RNA wt ] (t-1) •ρ + [RNA mt ] (t- 1) )•K 1 , where ρ is the probability of mutation during rep- lication and K 1 = e k . Therefore, while wild-type virus pre- dominates early, replication (and intracellular accumulation) of variant virus and viral proteins will accelerate (in a ratio of ([RNA wt ] (t-1) •ρ + [RNA mt ] (t-1) )/ [RNA wt ] (t-1) •(1-ρ) compared to wild type) and variant viral RNAs will rapidly predominate (Figure 1). Mutations progressively accumulate in RNA viruses [17] and ulti- mately variant RNAs and proteins, if variant RNAs are translated, will become dominant. It is also likely some variant viral proteins will resist cellular trafficking, further accelerating the intracellular accumulation of variant forms relative to wild type. The paradox of quasispecies stability Two fundamental problems critical to understanding RNA virus quasispecies biology arise because of RNA polymerase infidelity and the mode of viral replication: 1: Replication kinetics Hepatitis C, HIV, and HBV and other viruses, have broadly similar kinetics (Figure 2); initial high level viral replication that rapidly declines to relatively constant low- level viraemia [11,12], typically 2–3 logs lower than at peak, for prolonged periods, a kinetic profile attributed to "immune control" [12]. However, immune control is a conceptually problematic explanation for the initial decline in viral load; For example; why would potent host responses (of whatever type; humoral, cell mediated or intracellular immunity, or any combination thereof), hav- ing reduced viral load and antigenic diversity by a factor of 10 2–3 within days, falter once less than 1% of virus remains? Formally 1. Assume immune mechanisms reduce initial viral replication. 2. Let I c(t) represent the immune forces favouring viral clearance and V e(t) viral forces promoting quasispecies expansion pressures at time (t). 3. Assume immune pressures I c required to clear virus are proportional to viral concentration [V], that is; V e ∝ [V] (or V e = k e [V] where k e is some constant), so that I c required to clear one viral particle I c(1) is less than that I c required to clear 10 viral particles Ic (10) . 4. At equilibrium (e.g. time points B or C, Figure. 2) immune clearance pressures approximate viral antigenic expansion pressures: I c(b or c) ≈ V e(b or c) . Eq.1 Effect of RNApol fidelity on replicationFigure 1 Effect of RNApol fidelity on replication. Each replica- tion cycle may produce either wild-type (Wt) or variant (Mt) copies of parental template in a ratio determined by polymerase fidelity. If HCV RNA pol M u is 10 -5 mutations per base RNA synthesized, Mt:Wt ratio at G 1 is ~9:1, by G 3 unmutated parental genome is 6.8 × 10 -4 of total virus popula- tion, and by G 20 7.5 × 10 -22 P P P P P P P Wt Mt Mt Wt P P P P P Mt Mt Mt Mt Mt Mt G 1 G 2 G 3 Viral kinetic paradoxFigure 2 Viral kinetic paradox. Viral replication kinetics (—). If host factors (I c , black arrows) reduce viral replication acutely (point A), then they must exceed viral forces (V e , grey arrows). At equilibrium (e.g. points B or C) host forces must balance viral forces; I c must therefore fall by a factor of 10 2–3 from A. Viral levels (Arbitrary units) 0 10 100 1000 Days Months Time Years AB A B C Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 3 of 14 (page number not for citation purposes) 5. If I c causes the reduced viral load seen between time A and time B or C, [V e(a) ] ⇒ [V e(b or c) ], then immune clear- ance pressures must exceed viral expansion pressures at that time i.e. I c(a) > V e(a) . Eq.2 6. As viral antigenic expansion pressures at time A exceed those at time (B or C) by 10 2–3 [V (a) ] ≈ [V (b or c) ]• 10 2–3 , and I c(b or c) = V e(b or c) then immune clearance pressures at time A exceed those at time (B or C) by10 2–3 I c(a) >I c(b or c) • 10 2– 3 . That is, immune pressures fall by 10 2–3 between time A and B or C, (Figure. 2). Prompting i) Why, and by what mechanism, would immune forces, or any other host defense mechanisms, fall by 10 2–3 over days between time A and B or C? There is, of course, no evidence immune pressures fall, and very considerable evidence both antibody and adap- tive T cell responses are increasing when viral replication is falling [5,12]. These facts are irreconcilable with the notion that immune or other any host mechanisms con- trol initial viral replication and strongly suggest immune or any other host mechanism(s) are not the primary rea- son viral load falls initially. Further, as down-regulation of viral replication frequently occurs prior to development of neutralising antibody, in the absence of any demonstrable antiviral antibody, or T-cell responses [25,41], and without lysis of infected cells [25], it is difficult to argue, with any conviction, that either humoral or cellular immune responses primarily cause reduced viral replica- tion. Evidence that prior HCV infection does not confer protective immunity against either heterologous HCV infection in chimpanzee [22]or either homotypic [33] or heterotypic [32] human reinfection further undermines the paradigm of "immune control". Inhibition of immune or other host mechanisms is an untenable expla- nation of this massive apparent fall in immune clearance pressures; if occurred to any degree, an increase, rather than the observed decrease, in viremia would result. In the absence of a rational host mechanism consistent with observed viral kinetic data, the ineluctable conclusion is that non-host (i.e. viral) mechanisms (i.e. viral auto regu- lation) must be operative. Chronic viral persistence raises other issues; At steady state (e.g. points B or C, Figure. 2), the rate of HIV and HCV production is estimated at 10 10 molecules / day [11,29,52,57] while HBV production may be 10 11 mole- cules/day resulting in an average viral load of 10 10 mole- cules/person [52,57]. However, during peak replication virus production may 10 2–3 times the basal rate [11,12], indicating enormous reserve replicative capacity. As basal viral replication is clearly sufficient for long-term stability, and kinetic analysis suggests viral, rather than host, factors control viral replication, the following questions are posed: When challenged, how do viruses "sense" the threat and by what mechanism do they modulate replica- tion in response? Problem 2: Mutation rate The stability of RNA viral quasispecies poses a major prob- lem: During viral replication the copied genome may either identical to or a variant of parental template (Fig- ure. 1). The probability (ρ) of a mutation occurring during replication is a function of polymerase fidelity; During one replication cycle ρ = (1-(1-M µ ) n ), where (M µ ) is muta- tion rate and (n) genome size. Hepatitis C (a ~9200 bp RNA virus) RNA pol introduces mutation at 10 -5 substitu- tions/base, ρ≈0.912. However, for multiple (θ) replica- tions cycles, ρ = (1-(1-M µ ) n ) θ . After 20 replication cycles, occurring in <7 days in most patients [52,57], the proba- bility of any original genome remaining un-mutated is ρ o ≈7.5 × 10 -22 , meaning effective loss of sequence infor- mation, an outcome that should cause quasispecies extinction [16]. Persistence of stable RNA viral quasispe- cies is, therefore, highly paradoxical [18]. This "theoretical impossibility" of RNA quasispecies stability suggests either a) the consistently reported rates of RNA pol infidel- ity are incorrect (which, even if true, would only delay quasispecies extinction; if M µ = 10 -10 , ρ o <10 -40 within 100 days etc.) or b) that innate viral mechanism(s) control RNA pol fidelity and mediate selective replication of con- sensus sequence genomes. Thus, rates of viral mutation are tightly constrained by the necessity to retain sequence information. On the other hand, overly faithful template replication will restrict antigenic diversity, rendering virus susceptible to immune destruction and unresponsive to ongoing cellular changes. The necessity to retain sequence information by adequate replicative fidelity, and the later requirements (in terms of replicase ⇒ RNA pol evolution) of viruses to access cells via evolving cell receptors and evade host defence mechanisms, has placed constraints on replicase (RNA pol ) function that dictate polymerase fidelity must be tightly, and dynamically, controlled (Fig- ure 3a). Evolutionary constraints on viral replication Optimal viral replication is a compromise between max- imising host-to-host viral transmission at each host con- tact versus maximising transmission at sometime during the host's life: Uncontrolled, exponential growth, as might result from the mode of viral replication, would cause rapid cell lysis, host death and a reduced likelihood of stable host-to-host transmission, a prerequisite for viral survival on an evolutionary timescale. While maximising the probability of host-to-host transmission at each con- tact, high-level viral replication increases the probability of host disease, thus reducing opportunity for transmis- sion long term. Contrariwise, adverse viral outcomes may Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 4 of 14 (page number not for citation purposes) a. Constraints on viral mutationFigure 3 a. Constraints on viral mutation. Inadequate polymerase fidelity will cause loss of sequence information and quasispcies extinction (A, B), while inadequate viral mutation will result in immune recognition and viral clearance (D,E). Viral persistence requires polymerase fidelity responsive to the host environment (C). 3b. Constraints on viral replication. Overly rapid replication will cause cell lysis, tissue injury and premature host death (A,B), while inadequate replication will result viral latency or clearance (D,E). Viral persistence with optimal evolutionary stability requires a polymerase responsive to the host environment (C). M E M D M B M er M ic Mutation Rate Clearance Viral Extinction C A E B D Probability of Immune Clearance Probability of Fitness Loss Optimal Rate of Mutation Zone of Stable Mutation Zone of Stable Mutation Reduced Replicative Fitness Effective Immune Response R P R D R B R L R C Tissue Damage Replication Rate Viral Clearance Time Host Death Viral Latency A B C D E Optimal Replication Zone of Stable Replication Zone of Stable Replication Probability of Host Survival Probability of Virus Transmission 3A 3B Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 5 of 14 (page number not for citation purposes) result from inadequate viral replication causing increased clearance and reduced host-to-host transmission. Viruses that cause premature host death or that are cleared by host mechanisms before transmission to, and infection of, other hosts are biological failures that have strong Dar- winian pressures acting against them. Optimal long-term viral stability, therefore, dictates viral replication rates (that is, polymerase processivity) and mutation frequency (that is, polymerase fidelity) must be closely regulated (Figure 3b). Hypothesis That viruses capable of chronic persistence auto-regulate replication and mutation rates by replicative homeostasis. Replicative homeostasis results when RNA polymerase end-translation products (envelope and contiguously encoded accessory proteins) interact with RNA pol to alter processivity and fidelity. Evidence for Autoregulation Substantial clinical and in-vitro evidence, including the kinetic paradox indicate viruses auto-regulate. During successful antiviral treatment levels of virus fall sharply [12,29,52,53,57], often becoming undetectable. How- ever, viral replication rebounds, rapidly and precisely, to pre-treatment levels on drug withdrawal in patients [52,53,57] and in tissue culture [1]. This in-vitro data con- firm replication is controlled by factors independent of either cellular or humoral immune function. Auto-regula- tion of HCV replication was confirmed most emphatically in patients undergoing plasmapharesis in whom 60–90% reduction in levels of virus returned to baseline, but not beyond, within 3–6 hours of plasma exchange [44]. Stud- ies suggesting autoregulation of tobacco mosaic virus rep- lication occurred independent of interferon effects, intrinsic interference or interference by defective virus [34] confirming this phenomenon is not confined to either animal viruses or cells. These data beg the ques- tions: How does the replicative mechanism "choose" any particular level of replication and how does it return, so accurately, to pre-treatment levels? RNA polymerase control Most cellular enzymes are under some form of kinetic control, usually by product inhibition. While simple neg- ative-feedback product inhibition is sufficient to control enzyme reaction velocity and the rate of product synthe- sis, it is inadequate to ensure the functional quality of any complex molecules – including proteins – synthesised. The functionality of RNA pol output depends on the func- tionality of protein(s) translated from any RNA synthe- sized by RNApol. For viruses, and their polymerase, evolutionary survival – i.e. whether the polymerase, and its viral shell, avoids immune surveillance, gains access to cells, and replicates to infect other hosts – is a function of the properties that the sequence, topological variability and structural integrity of envelope proteins impart. RNA polymerase is responsive to and is influenced by accessory proteins that induce conformational changes to alter both processivity and fidelity [20,31], representing partial "proof of concept" of the mechanism postulated. Evolutionary stability Evolutionary stability requires adaptability to changing environmental circumstances. For viruses, an ability to modulate replication and mutation rates dynamically in response to cellular changes is essential. Viruses intrinsi- cally capable of adaptation to environmental changes, including variations in host density, and evolving cell receptor polymorphisms, immune and other host responses, among other variables, will enjoy a competi- tive advantage over viruses lacking innate responsiveness. Contrariwise, self-replicating molecules, including viruses, that lack innate adaptability, for whom replica- tion is contingent upon a chance confluence of appropri- ate cellular conditions – including permissive cell receptors, absence of cell defences and so on – are highly vulnerable to extinction by both adverse environmental changes and competition for scarce intracellular resources by molecules capable of adaptation. For viruses, this adaptability requires antigenic and structural diversity be controlled and, in turn, that means the two critical RNA pol attributes, fidelity and processivity, be dynamically modi- fiable, and controllable. These linked functional require- ments imply a dynamic nexus between the functional output of RNA pol (i.e. envelope proteins) and that polymerase. Homeostatic systems Systems capable of homeostatic regulation (auto-regula- tion) have the following characteristics: i) an efferent arm that effects changes in response to perturbations of an equilibrium; ii) an afferent arm that measures the systems response to those changes; iii) mechanism(s) by which i) and ii) communicate. The mechanism of viral autoregula- tion – Replicative Homesostasis – described here requires: i) that viral envelope (Env) proteins interact with viral RNA polymerases (RNA Pol ); ii) that these Env :RNA Pol interactions alter both polymerase processivity and fidel- ity; iii) that wild-type (consensus sequence) Env wt :RNA Pol complexes cause more rapid, less faithful RNA replication than variant (variant) Env mt :RNA Pol complexes. There is solid evidence for each requirements of replicative homeostasis. The Envelope-Polymerase relationship: Evidence for mechanism A large body of literature, for many viruses, establishes an important relationship between envelope and polymerase Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 6 of 14 (page number not for citation purposes) proteins and documents that Env proteins influence both RNA Pol processivity and fidelity. First, for HIV, overwhelming evidence suggests HIV polymerases properties, and those of related retroviruses – for example, simian immunodeficiency virus (SIV) and the feline immunodeficiency virus (FIV) – are influenced by Env proteins (for example, [9,15,35]. Broadly, these indicate heterologous Env proteins – when administered as live attenuated vaccines [71], adjuvant enhanced pro- tein vaccine [83], or as recombinant Env proteins in cell culture [64] – dramatically alter viral load, and both rep- lication and mutation rates of wild-type virus. Specific examples include data demonstrating HIV Env regions obtained from different patient isolates, when cloned into common HIV-1 backbones, conferred a spectrum of repli- cation kinetics and cytotropisms characteristic of the orig- inal Env clone, and independent of either the clones' ability to raise antibody [51], or the replicative character- istics of the 'native' polymerase backbone [51]. Similarly, chimeric HIV-1 viruses expressing heterologous Env, again with a common polymerase backbone, have replica- tion kinetics and cell tropism phenotypes identical to the parental Env clone [39], suggesting the Env is a critical determinant of polymerase function. Similar results obtained with SIV clones [36] strongly support conclu- sions drawn from feline immunodeficiency virus [37] data. Fine mapping of HIV envelope proteins identified 6 mutations within the V1-V3 loop that increased viral replication in a manner independent of nef [77], confirm- ing other work examining HIV Env recombinants [14], and extending earlier work that demonstrated a single amino acid substitution (at position 32 of the V3 Env domain) was sufficient to change a low replication phe- notype into high-replicating phenotype [13]. Finally, for HIV, co-transfection with Env variants at 10 fold excess dramatically inhibited replication of wild-type virus [75], providing direct evidence for both the interaction and dif- ferential affinity for wild-type and variant Env for polymerases. Critically, many of these observations are from in-vitro systems, indicating the effects are independ- ent of either cellular or humoral immune influence. Many studies report the effect of Env/polymerase interactions in terms of altered viral tropisms, and did not examine changes to polymerase fidelity explicitly. However, virus replication can alter in only two ways; either there is more or less virus, or the viral genomic sequence may be changed by altered polymerase fidelity. Variant viruses expressing altered envelope proteins will have altered cell receptor affinities and hence, variable cell tropisms. Second, for HCV, many separate observations document HCV replication and polymerase functionality is depend- ent on envelope proteins: i) HCV viral genotypes are defined by sequences of either envelope or polymerase regions [43,73,74] and these are necessarily acquired together – a genetic nexus implying a functional relation- ship. ii) Observations that a) co-infection with multiple HCV genotypes occurs less frequently than predicted by chance and b) certain HCV genotypes become progres- sively dominant in populations both suggest – at a popu- lation level – replicative suppression of some HCV genotypes by others [68]. These observations are sup- ported by observations of both homotypic [33] and heter- otypic HCV super-infection [32] documenting genotype- dependent replicative suppression of one HCV genotype by another in individual patients. iii) Functional infec- tious chimeric viruses with polymerase and Env proteins derived from different genotypes have not been reported. iv) Full-length HCV chimeras, engineered with deletions of p7 envelope proteins, are replication deficient and non- infections, indicating intact genotype-specific HCV enve- lope sequences are essential for proper HCV replication. Specific replacement of p7 of the 1a clone with p7 from an infectious genotype 2a clone was replication defective, suggesting a genotype-specific interaction between the p7 envelope protein and other genomic regions [66]. v) In two independent chimpanzees studies HCV inoculation resulted in persistent infection only in animals developing anti-envelope (E2) antibodies, whereas failure to produce anti-E2 was associated with viral clearance [4,62], intui- tively a highly paradoxical result difficult to rationalize unless E2 proteins are important for sustained HCV repli- cation, as we argued previously [45]. vi) Finally, for HCV, specific motifs within the [polymerase] NS5 region of HCV in chronically infected patients predict response to interferon [19,67] an observation that makes little sense unless interferon interacts directly with NS5 [polymerase] motifs, as in-vitro studies suggest [10]. Third, HBV envelope and polymerase protein genes have overlapping open reading frames and significant altera- tions in envelope and polymerase gene and protein sequences cannot, therefore, occur independently, a genetic nexus again implying an important functional relationship. Mutations in envelope sequences occurring spontaneously [82] following therapy of HBV with lamu- vidine and immunoglobulin prophylaxis [6,72] or after vaccine escape [8] are frequently associated with high level viral replication, although replication-deficient mutations are described [47]. These data are generally interpreted to mean polymerase gene mutation(s) cause altered polymerase protein sequence and, hence, abnor- mal polymerase function. While this is probably partially true if the functionally relevant HBV RNA polymerase is an envelope/polymerase heterodimer (analogous to the p66/p51heterodimer of HIV RT [30]), then an equally valid interpretation is that mutations in envelope genes may change envelope protein conformation and therefore alter normal envelope/polymerase interactions, thus Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 7 of 14 (page number not for citation purposes) altering processivity and fidelity of the replication com- plex. This latter interpretation is convincingly supported by data demonstrating that abnormal polymerase func- tion of HBV envelope variants is reversed by co-transfec- tion of Hep G2 cells with clones expressing wild-type envelope sequences [81] and is further supported by clin- ical studies demonstrating administration of exogenous HBsAg (protein) to patients with chronic HBV dramati- cally reduced HBV replication [60]. Fourth, studies of the coliphage Qβ demonstrate phage coat proteins bind to genomic RNA [86]to strongly inhibit (association K ic ≈ 10 7–8 M -1 , inhibition K i ≈ 10 9 M -1 s -1 ) [79] RNA replication by direct suppression of polymerase activity by envelope proteins [18]. This interaction is dependent on the binding site conformation, but not RNA sequence[86], suggesting interaction avidity will vary as an inverse function of protein sequence divergence from wild type, an intuitive expectation confirmed exper- imentally [79]. An impressive body of literature documents similar relationships between envelope and polymerase function in swine fever, tobacco mosaic [34], brome mosaic [2] and other RNA viruses. Importantly, studies of the tobacco mosaic virus confirmed this effect to be host-independent and virus-specific inhibition of viral RNA synthesis and to be quite distinct from any interferon effects, intrinsic interference or interference by defective virus [34]. Thus, there exists solid evidence for each necessary component of replicative homeostasis for HCV, HBV and HIV, and other viruses. Replicative homeostasis: proposed mechanism Replicative homeosatsis results from differential interac- tions of wild-type (Wt) and variant (Mt) envelope pro- teins on RNA pol in a series of feedback epicycles linking RNA pol function, RNA replication and protein synthesis (Figure 4, 5). Intracellular accumulation of variant viral proteins causes progressive, direct, inhibition of RNA pol and also block Env Wt :RNA pol interactions that increase replication and mutation. Progressive blockade of RNA pol by variant envelope results in a less processive, more faith- ful, polymerase, increasing the relative output of wild- type envelope RNAs, and, subsequently, translation of wild-type envelope proteins and, hence, an inexorable progression to stable equilibria. Quasispecies stability, and other consequences (including immune escape and low-level basal replication), are inevitable outcomes that result from equilibria reached because of these interac- tions (Figure 5). We suggest these interactions, and the resulting equilibria, are important therapeutic targets, and the effective ligands – envelope proteins or topologically homologous molecules – implicit within this hypothesis. Viral polymerases are clearly the effector mechanism – the efferent arm – that determines rate of viral RNA replica- tion and mutation. The afferent arm needs to measure both the rate of viral replication and degree of viral muta- tion. Intracellular envelope concentrations are a direct function of effective viral replication, while competition between wild-type and variant envelope proteins for inter- action with RNA pol allows determination of viral muta- tion rates. Envelope proteins, as opposed to other viral products, are the obvious products to examine for func- tional variability, and must form part of the afferent arm necessary to "sense" perturbations in the viral equilib- rium. While other viral products could be "sensed" to gauge effective viral replication, only functional measure- ment of envelope protein concentration and topological variability simultaneous measures both the rate of viral replication and envelope functions – properties deter- mined by envelope structure and antigenic diversity – essential for viral survival; immune escape and cell access. Furthermore, envelope and polymerase proteins are typi- cally coded at transcriptionally opposite ends of the viral genome; replication contingent upon a dynamic nexus between envelope and polymerase proteins is, therefore, a Mechanism of replicative homeostasisFigure 4 Mechanism of replicative homeostasis. At A, relatively high concentrations of Env Wt (blue, A) favour high affinity Env:RNA pol interactions out-competing variant forms (Env mt , red), increasing RNA pol processivity but reduced fidelity increasing relative output of variant RNAs. Subsequent ribos- omal (R, mauve) translation increases concentrations Env mt (red), relative to Env Wt , returning the system to equilibrium. Relative excess Env mt (B, red) out-compete Env Wt (blue) for interactions with RNA pol , favouring Env mt :RNA pol , and block- ing Env Wt :RNA pol interactions. Env mt :RNA pol complexes rela- tively decrease RNA pol processivity but increase fidelity, increasing output of wild-type RNAs. Subsequent increased translation of Env Wt relative to Env mt restores the equilibrium. R POL (A) POL (B) R Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 8 of 14 (page number not for citation purposes) Conseqences of replicative homeostatic cyclesFigure 5 Conseqences of replicative homeostatic cycles. Disturbance to intracellular replicative homeostatic cycles. Events increasing intracellular Env Wt : Env mt ratio (exogenous addition of Env Wt , antibody recognition of Env mt ) will favour Env Wt :RNA pol interactions, increasing RNA pol processivity and reducing fidelity increasing relative output of variant virus. Con- versely, events decreasing intracellular Env Wt : Env mt ratios (exogenous addition of Env mt , antibody recognition of Env Wt ) will favour Env mt :RNA pol interactions, decreasing RNA pol processivity and increasing fidelity, thus reducing replication. env 1 2 3 4 (B) R R POL POL Env Env Env Env Env Env (A) Env Env Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 9 of 14 (page number not for citation purposes) functional check of the integrity of the entire viral genome. Importantly, this facet of replicative homeostasis is a direct mechanism of Darwinian selection operating at a molecular level, that ensurs preferential selection and replication of "fit" viral genomes, and maintenance of genotypes (species). Viruses, notably HIV, produce many accessory proteins (such as HIV Nef, gag, rev and HBeAg) that affect viral rep- lication and mutation rate. However, these proteins are encoded within envelope open reading frames (ORFs) or are contiguous with them and are likely to alter function- ally with any mutation affecting envelope sequences (Fig- ure 6). While these accessory proteins may interact with RNA pol (with or without Env) to reset replicative equilib- rium (by changing replication rate or mutation frequency or both), stable equilibria will still result providing the sum effect of variant proteins encoded within the enve- lope ORF is to decrease RNA pol processivity (v) and muta- tion (M u ) frequency relative to wild-type protein polymerase interactions. Testing the hypothesis This hypothesis is simply tested. Manoeuvres that increase intracellular concentrations of variant envelope proteins or decrease wild-type envelope proteins should inhibit viral replication and reduce mutation rates. Conversely, manoeuvres increasing intracellular [Env Wt ] or reducing intracellular [Env mt ] should accelerate viral replication and mutation. In fact, observations relevant to every aspect of this hypothesis have been reported in a variety of systems and circumstances. All outcomes are completely consistent with those predicted by replicative homeosta- sis. Replicative homeostasis predicts, for example, HCV E2 proteins derived from genotype 1 HCV sequences would reduce HCV replication when administered to patients with heterologous HCV infection (genotypes 2,3 or 4, for example) and studies examining heterologous envelope proteins as direct RNA pol inhibitors are underway. Discussion Replicative homeostasis immediately resolves the paradox RNA viral quasispecies stability and explains how these viruses persist and, thereby, cause disease. Replicative homeostasis also explains the initial decline of viral repli- cation, resolving the kinetic paradox, rationalizing the dynamics of chronic viral infection and other enigmatic and unresolved viral behaviours. Most importantly, repli- cative homeostasis implies a general approach to antiviral therapy. The equilibria formed by replicative homeostasis are responsive to disturbance of envelope concentrations ensuring viral mutation is neither random nor passive but highly reactive to external influence: Sustained reduction of viral envelope (by immune or other mechanisms) would favour high affinity Env Wt : RNA pol interactions that, in turn, increase polymerase processivity but reduce fidel- ity accelerating synthesis of variant viral RNAs and, conse- quently, increased translation of antigenically diverse proteins, reactively driving quasispecies expansion and generating the extreme antigenic diversity of RNA quasispecies. Alternatively, in the absence of immunolog- ical recognition, variant envelope / polymerase interac- tions predominate, restricting viral replication and mutation, thus maintaining basal output of consensus viral sequences, thus maintaining genotype. Immune escape and maximal cell tropism are inevitable conse- quences of the potential antigenic diversity generated by RNA replication mediated by the reactive equilibria of replicative homeostasis. Potential viral antigenic diversity is numerical superior to any immune response; Theoretically, a small envelope protein of 20 amino acids could assume 20 20 (about 10 26 ) possible conformations, greatly exceeding the ~10 10 anti- body [80] or CTL receptor conformations either humoral and cellular immune responses can generate. A direct consequence of this mismatch and the stable reactive, equilibria resulting from replicative homeostasis is that once infection is established, the clinical outcome is pri- marily determined by the viruses' ability to maintain control of the quasispecies, rather than the hosts' response to that quasispecies. This sanguine view is supported by both general clinical experience and by kinetic analysis of chronic viral infection (Figure 2); if host responses are unable to clear virus at 10 5–7 viral equivalents / ml they are not likely to be any more effective at 10 8–11 eq/ ml. The varied clinical outcomes of viral infections are explained by replicative homeostasis and its failure: Viral failure to down-regulate replication by RNA pol inhibition would cause rapidly progressive or fulminant disease (characterised by massively polyclonal, but ultimately ineffectual, immune responses), while inadequate replica- tion or generation of diversity will result in viral clearance (Figure 3b). Stable, homeostatic replicative equilibria will result in chronic infection with episodic fluctuations in viral replication and host responses (eg ALT; [65]) typical of chronic hepatitis or HIV. The widely varied spectrum and tempo of viral diseases, that for viral hepatitis ranges from asymptomatic healthy chronic carriage to fulminant liver disease and death within days, is far more rationally explained on the basis of a broad spectrum of polymerase properties than highly variable and unpredictable (yet genetically homogeneous) immune responses. Homeostatic systems functioning without external pertur- bations – such as thermostatically controlled water tanks – progress rapidly to stasis (Figure 7). In tissue culture, Virology Journal 2005, 2:10 http://www.virologyj.com/content/2/1/10 Page 10 of 14 (page number not for citation purposes) Phenotypic effects of RNA quasispecies complexityFigure 6 Phenotypic effects of RNA quasispecies complexity. Two-dimensional representation of multi-dimensional hyperdense sequence-space that define viral quasispecies; vast RNA /proteins populations progressively divergent from consensus sequence (0). As genetic the distance of RNAs increases from consensus sequence the amino acid sequence, conformation, and functional properties of resulting proteins may also change, potentially resulting in proteins that, despite originating from iden- tical [consensus sequence] genetic domains, have diametrically opposed function. As many accessory proteins (for example, HIV rev, tat, nef and HCV HP7) have open reading frames contiguous with Envelope, sequence changes to Env will also affect accessory protein function. 0 Consensus Sequence R R R R R rev tat nef rev tat nef env env + – HCV P7 HCV P7 R R [...]... killer cell activation and antibodydependent cellular cytotoxicity by interferon-alpha and interleukin-12 in vaginal mucosae Sivmac251-infected Macaca fascicularis Viral Immunol 2002, 15:197-212 Pol S: Immunotherapy of chronic hepatitis < /b> B by anti HBV vaccine Biomed Pharmacother 1995, 49:105-9 Preston BD, Poiesz BJ, Loeb LA: Fidelity of HIV-1 reverse transcriptase Science 1988, 242:1168-71 Prince AM, Brotman... 28:71-6 Publish with Bio Med Central and every scientist can read your work free of charge "BioMed Central will be the most significant development for disseminating the results of biomedical researc h in our lifetime ." < /b> Sir Paul Nurse, Cancer Research UK Your research papers will be: available free of charge to the entire biomedical community peer reviewed and published immediately upon acceptance cited... encephalitis[84], Ebola [78] Coxsackie [24] and other viruses Similarly, increased HIV replication and mutation after influenza [38] or tetanus [56] vaccination; reduced HIV replication during measles [50] and Dengue [85] co-infection; clearance of HBV without hepatocyte lysis or evidence of T cell dependent cytotoxicity[25], are also explained by this mechanism Previously unexplained and problematic... Klaver B, Krone W, Tersmette M, de Ronde A: Human immunodeficiency virus type 1 clones chimeric for the envelope V3 domain differ in syncytium formation and replication capacity J Virol 1992, 66:757-65 DeStefano JJ: Interaction of human immunodeficiency virus nucleocapsid protein with a structure mimicking a replication intermediate Effects on stability, reverse transcriptase binding, and strand transfer... explain both the genotype specificity of interferon action and the kinetics of action and, incidentally, the apparent "immune enhancement" [59] caused by interferon; if interferon reduces RNApol processivity while increasing its fidelity, viral RNAs synthesized will contain fewer mutations causing synthesis of antigenically restricted proteins, thus presenting a more homogeneous target susceptible to... Locarnini SA, Manns M, Trautwein C,< /b> Bock TC: Restoration of replication phenotype of lamivudine-resistant hepatitis < /b> B virus mutants by compensatory changes in the "fingers" subdomain of the viral polymerase selected as a consequence of mutations in the overlapping S gene Virology 2002, 299:88-99 Tran A, Kremsdorf D, Capel F, Housset C,< /b> Dauguet C,< /b> Petit MA, Brechot C:< /b> Emergence of and takeover by hepatitis.< /b> .. of "rival" genes, are strongly selected for, and are highly conserved in evolution The interferons, and other cytokines, are cellular defence mechanisms that long antedate the immune system If the interferons are functionally homologous to viral envelope proteins, and interact with viral RNApol to reduce processivity and replication to restrict viral replication and antigenic diversity, increasing their... polymerases activity are strongly conserved in evolution, suggesting a critical cellular function Control of DNAdependent RNApol transcription by DNA viruses, cellular micro-organisms (e.g malaria), and eukaryotic cells, subtly modulating cell-surface protein expression, via replicative homeostasis, to mediate immune escape, control cell division and differentiation, or other functions would not be surprising... Tanzi E, Zuckerman AJ, Thomas HC: Vaccine-induced escape mutant of hepatitis < /b> B virus Lancet 1990, 336:325-9 Chen M, Shi C,< /b> Kalia V, Tencza SB, Montelaro RC, Gupta P: HIV gp120 V(1)/V(2) and C(< /b> 2)-V(3) domains glycoprotein compatibility is required for viral replication Virus Res 2001, 79:91-101 Chung RT, He W, Saquib A, Contreras AM, Xavier RJ, Chawla A, Wang TC, Schmidt EV: Hepatitis < /b> C < /b> virus replication... Broom AK, Mackenzie JS, Hall RA, Shellam GR, McMinn PC: Antibody-dependent enhancement of Murray Valley encephalitis virus virulence in mice J Gen Virol 2003, 84:1723-8 Watt G, Kantipong P, Jongsakul K: Decrease in human immunodeficiency virus type 1 load during acute dengue fever Clin Infect Dis 2003, 36:1067-9 Witherell GW, Uhlenbeck OC: Specific RNA binding by Q beta coat protein Biochemistry 1989, . Abstract Hepatitis C (HCV), hepatitis B (HBV), the human immunodeficiency viruses (HIV), and other viruses that replicate via RNA intermediaries, cause an enormous burden of disease and premature death. fever, tobacco mosaic [34], brome mosaic [2] and other RNA viruses. Importantly, studies of the tobacco mosaic virus confirmed this effect to be host-independent and virus-specific inhibition of viral. when cloned into common HIV-1 backbones, conferred a spectrum of repli- cation kinetics and cytotropisms characteristic of the orig- inal Env clone, and independent of either the clones' ability